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UPTAKE OF THYROXINE IN CULTURED ANTERIOR-PITUITARY-CELLS OF EUTHYROIDRATS

Authors

EVERTS ME DOCTER R MOERINGS EPCM VANKOETSVELD PM VISSER TJ DEJONG M KRENNING EP HENNEMANN G

Citation

Me. Everts et al., UPTAKE OF THYROXINE IN CULTURED ANTERIOR-PITUITARY-CELLS OF EUTHYROIDRATS, Endocrinology, 134(6), 1994, pp. 2490-2497

Citations number

Categorie Soggetti

Endocrynology & Metabolism

Journal title

Endocrinology → ACNP

ISSN journal

00137227

Volume

134

Issue

Year of publication

1994

Pages

2490 - 2497

Database

ISI

SICI code

0013-7227(1994)134:6<2490:UOTICA>2.0.ZU;2-#

Abstract

The uptake of [I-125]T-4 was investigated in cultured anterior pituita ry cells isolated from adult fed Wister rats and cultured for 3 days i n medium containing 10% fetal calf serum. Experiments were performed w ith [I-125]T-4 (10(5) to 2 x 10(6) cpm; 0.35-7 nM) in medium containin g 0.5% or 0.1% BSA. The uptake of [I-125]T-4 increased with time and s howed equilibrium after around 1 h of incubation. The presence of 10 m u M unlabeled T-4 during incubation decreased the uptake of [I-125]T-4 by 65-70% at all time intervals. After 24 h of incubation, 1.5% iodid e and 3.2% conjugates were detected in the medium, whereas around 20% of cellular radioactivity represented [I-125]T-3. The 15-min uptake of [I-125]T-4 was significantly reduced by simultaneous incubation with 100 nM T-4 (by 24%; P < 0.05), 100 nM T-3 (by 38%; P < 0.001), or 10 m u M rT(3) (by 32%; P < 0.001), whereas 10 mu M tetraiodothyroacetic ac id (Tetrac) had no effect. Furthermore, preincubation (30 min) and inc ubation (15 min) with 10 mu M monodansylcadaverine, oligomycin, or mon ensin reduced the uptake of [I-125]T-4 by 30%, 50%, and 40%, respectiv ely (all P < 0.001). Substitution of Na+ in the buffer by K+ diminishe d the uptake of [I-125]T-4 by 39% (P < 0.005); 2 mM phenylalanine, tyr osine, or tryptophan reduced [I-125]T-4 uptake by 18% (P < 0.05), 18% (P = NS), and 33% (P < 0.005), respectively. Our data suggest that the pituitary contains a specific carrier-mediated energy-requiring mecha nism for [I-125]T-4 uptake that is partly dependent on the Na+ gradien t. In addition, part of [I-125]T-4 uptake in the pituitary might occur through an amino acid transport system. When expressed per pM of free hormone, the 15-min uptake of [(I-125]T-4 was approximately as high a s that of [I-125]T-3. Because the reduction of [I-125]T-4 uptake by T- 4, T-3, monodansylcadaverine, oligomycin, and monensin was roughly the same as the previously reported reduction of [I-125]T-3 uptake by the same compounds, it is further suggested that T-4 and T-3 Share a comm on carrier in cultured anterior pituitary cells.